Enhanced cell-free synthesis of active proteins containing disulfide bonds
a technology of disulfide bonds and active proteins, which is applied in the field of enhanced cell-free synthesis of active proteins containing disulfide bonds, can solve the problems of complex expression of mammalian proteins, difficulty in refolding of aggregated proteins, and high protein synthesis rate, so as to accelerate the rate-limiting covalent steps of folding and stabilize the redox potential of reaction mixes. , the effect of accelerating the rate-limiting covalent steps
Active Publication Date: 2008-10-09
THE BOARD OF TRUSTEES OF THE LELAND STANFORD JUNIOR UNIV
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Benefits of technology
[0020]In addition to stabilizing the redox potential of the reaction mix, the in vitro synthesis may be further enhanced by the inclusion of accessory proteins that assist in the proper folding of proteins in vivo. Of particular interest is the inclusion of foldases, proteins with a catalytic activity that serve to accelerate rate-limiting covalent steps in folding, e.g. PDI, dsbC, Skp, etc. Other modifications of interest include performing the reactions in the substantial absence of polyethylene glycol, which may be replaced with, e.g. spermidine, spermine, putrescine, and the like. The temperature at which the reaction takes place may be optimized for the protein, e.g. by reducing the temperature to about 25°, about 30°, about 32°, about 35°, about 37°, and the like.
Problems solved by technology
However, a high rate of protein synthesis is necessary, but by no means sufficient, for the efficient production of active biomolecules.
But although the formation of inclusion bodies can sometimes ease the purification of expressed proteins; in most occasions, refolding of the aggregated proteins remains a challenge.
These kinetic limitations result in the accumulation of partially folded intermediates that contain exposed hydrophobic ‘sticky’ surfaces which promote self-association and formation of aggregates.
Expression of mammalian proteins is more complicated than bacterial proteins because many of them require intramolecular disulfide bonds for their activity.
Even though the periplasmic space of Escherichia coli provides an oxidizing environment as well as folding proteins such as DsbA, B, C, and D, in many cases, simple secretion of complex proteins into the periplasmic space is not sufficient to form correct disulfide bonds.
However, the effect of molecular chaperones can be product-specific and the co-expression of each molecular chaperone with the target proteins is often cumbersome.
Moreover, in some cases, the expression of a molecular chaperone is detrimental to cell growth.
Despite the recent advances, the expression of properly folded mammalian proteins in Escherichia coli still remains as a great challenge.
This is mainly due to the difficulties in the control of the key parameters for disulfide bond formation including the sulfhydryl redox potential inside the cells.
In addition, removing the need to maintain host cell viability allows the production of proteins that are toxic to the host cell.
Unfortunately, GSSG is rapidly reduced during in vitro synthesis reactions by two enzymatic pathways mediated by glutathione reductase (Gor) and thioredoxin reductase (TrxB).
While IAM-mediated inactivation of TrxB and Gor is useful for promoting disulfide bond formation, conventional IAM treatment can also result in a reduction in protein yields (Kim and Swartz (2004) Biotechnol Bioeng 85:122-9).
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Materials and Methods
[0097]Construction of the KGK10 Strain. The objective here was to delete the gene encoding glutathione reductase (Gor) and to add the coding sequence for a hemagglutinin tag (HA Tag) to the trxB gene. For the latter, a PCR cassette was generated using the primers TrxB-HAFor (5′-tgatgcggaacgctacctcgatggtttagctgacgcaaaatacccatatgacgtcccggactacgcctaataaGTGTAG GCTGGAGCTGCTTC) and TrxB-HARev (5′-gtcgcatggtgtcgccttctttacttttgttactgatttCA TATGAATATCCTCCTTAGT) with the pKD3 plasmid template as described (Datsenko and Wanner (2000) Proc Natl Acad Sci USA 97:6640-5). In these primers, regions of homology are shown in lower case, the HA tag sequence is underlined, stop codons are in bold, and regions that anneal to the pKD3 plasmid are in capital letters. The cassette was transformed into the BW25113 pDK46 strain and selected on LB-Chloramphenicol. P1 bacteriophage transduction was used to move the genomic modification from a successful recombinant into KC6. FLP recombinas...
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Abstract
Compositions and methods are provided for the enhanced in vitro synthesis of active polypeptides containing disulfide bonds. In certain embodiments of the invention, the reaction mix includes a biological extract derived from a bacterial cell in which the glutathione reductase gene has been inactivated, which is pre-treated with a low concentration of a sulfhydryl inactivating agent.
Description
BACKGROUND OF THE INVENTION[0001]Escherichia coli is a widely used organism for the expression of heterologous proteins. It easily grows to a high cell density on inexpensive substrates to provide excellent volumetric and economic productivities. Well established genetic techniques and various expression vectors further justify the use of Escherichia coli as a production host. However, a high rate of protein synthesis is necessary, but by no means sufficient, for the efficient production of active biomolecules. In order to be biologically active, the polypeptide chain has to fold into the correct native three-dimensional structure, including the appropriate formation of disulfide bonds.[0002]In many cases, the recombinant polypeptides have been found to be sequestered within large refractile aggregates known as inclusion bodies. Active proteins can be recovered from inclusion bodies through a cycle of denaturant-induced solubilization of the aggregates followed by removal of the den...
Claims
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IPC IPC(8): C12P21/04C07K1/00
CPCC12P21/02
Inventor KNAPP, KURTIS G.SWARTS, JAMES ROBERT
Owner THE BOARD OF TRUSTEES OF THE LELAND STANFORD JUNIOR UNIV
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